WO2012128082A1 - Anti-mouse aggrus monoclonal antibody - Google Patents

Anti-mouse aggrus monoclonal antibody Download PDF

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WO2012128082A1
WO2012128082A1 PCT/JP2012/056142 JP2012056142W WO2012128082A1 WO 2012128082 A1 WO2012128082 A1 WO 2012128082A1 JP 2012056142 W JP2012056142 W JP 2012056142W WO 2012128082 A1 WO2012128082 A1 WO 2012128082A1
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antibody
aggrus
ferm
monoclonal antibody
human
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PCT/JP2012/056142
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Japanese (ja)
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直也 藤田
侑也 中澤
高木 聡
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公益財団法人がん研究会
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Priority to CN201280024485.7A priority Critical patent/CN104093741B/en
Priority to EP12760065.8A priority patent/EP2690111B1/en
Priority to US14/006,498 priority patent/US8980264B2/en
Priority to ES12760065.8T priority patent/ES2566133T3/en
Priority to KR1020137027784A priority patent/KR101956566B1/en
Priority to CA2836007A priority patent/CA2836007C/en
Priority to JP2013505892A priority patent/JP6218603B2/en
Publication of WO2012128082A1 publication Critical patent/WO2012128082A1/en

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    • C07K2317/34Identification of a linear epitope shorter than 20 amino acid residues or of a conformational epitope defined by amino acid residues

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  • the present invention relates to a mouse anti-Aggrus monoclonal antibody.
  • Platelet aggregation-inducing factor Aggrus (also known as podoplanin, gp44, etc.) is a type I transmembrane protein that is upregulated in various types of cancers such as squamous cell carcinoma, mesothelioma, Kaposi's sarcoma, testicular tumor and brain tumor. (Non-Patent Documents 1 to 9). There is a report that overexpression of Aggrus is associated with poor prognosis, suggesting an important involvement of Aggrus in cancer progression (Non-Patent Documents 10 and 11). It is known that the expression of Aggrus causes platelet aggregation and promotes experimental and spontaneous lung metastasis in mice (Non-patent Documents 11 and 12).
  • Non-patent Documents 11 and 12 Cancer cell-induced platelet aggregation is thought to form large cancer-platelet aggregation, leading to increased embolization of cancer cells in the microvasculature and protection from immunological attack in the circulation. Recently, a C-type lectin-like receptor (CLEC-2) expressed on platelets has been identified as one of the Aggrus counterpart receptors.
  • CLEC-2 C-type lectin-like receptor
  • Non-patent Document 13 It is known that when CLEC-2 binds to Aggrus expressed on tumor cells, an activation signal is produced in platelets without plasma components, and triggers platelet aggregation.
  • the domains of Aggrus and CLEC-2 that are critical for mutual recognition are already known (Non-patent Document 13).
  • Monoclonal antibodies can bind specifically and specifically to cell surface antigens and cause an immunological response to target cells. Therefore, many monoclonal antibodies are currently used for cancer treatment. There are three typical monoclonal antibodies used in cancer treatment: neutralization, antibody-dependent cytotoxicity (antibody-dependent cellular cytotoxicity; ADCC) and complement-dependent cytotoxicity (complement-dependent cytotoxicity; CDC). Shows anticancer effects through its mode of action. Antibodies, such as bevacizumab and cetuximab, can inhibit ligand-receptor binding or receptor multimerization and neutralize signal pathway activation. Since the growth of cancer cells depends on the activation of the signal pathway, neutralization thereof leads to cell death.
  • the antibody can induce an immune response against the target cancer cell via its Fc domain.
  • Effector cells and complements such as macrophages, NK cells, and neutrophils recognize the Fc domain of antibodies that bind to cancer-specific antigens and consequently kill the target cancer cells.
  • An object of the present invention is to provide a pharmaceutical composition for treating cancer and thrombosis with Aggrus as a target.
  • the present invention provides a fragment (1) comprising a mouse monoclonal antibody or a functional fragment thereof that recognizes an Aggrus epitope comprising the amino acid sequence represented by SEQ ID NO: 1, 3, or 4.
  • the present invention also relates to a fragment comprising the monoclonal antibody according to the above (1) or a functional fragment thereof produced by a hybridoma of accession number FERM BP-11446, FERM BP-11447, FERM BP-11448 or FERM BP-11449.
  • the present invention provides a humanized fragment (3) comprising the monoclonal antibody according to (1) or (2) or a functional fragment thereof.
  • the present invention also provides the pharmaceutical composition (7) according to the above (6), wherein the thrombosis is cerebral infarction or myocardial infarction. Furthermore, the present invention provides the pharmaceutical composition (8) according to (6) above, wherein the cancer or tumor is squamous cell carcinoma, fibrosarcoma, mesothelioma, Kaposi sarcoma, testicular tumor, brain tumor or bladder cancer. . Preferably, the present invention provides the pharmaceutical composition (9) described in (8) above, wherein the cancer or tumor is squamous cell carcinoma, mesothelioma, testicular tumor or bladder cancer.
  • the mouse monoclonal antibodies designated P2-0, MS-1, MS-3, and MS-4 produced from the hybridoma established by the present inventors were analyzed in vivo and in vitro. It was found that the epitope of Aggrus consisting of the amino acid sequence represented by 3 or 4 was recognized, and binding of Aggrus-CLEC-2 was inhibited in a concentration-dependent manner.
  • the monoclonal antibody of the present invention also showed an effect of suppressing platelet aggregation and an effect of suppressing lung metastasis of cancer.
  • the humanized antibody (human chimeric antibody) of the monoclonal antibody of the present invention showed an effect of suppressing cancer metastasis even in cells with low expression of Aggrus.
  • the monoclonal antibody of the present invention is different in reactivity to native Aggrus expressed in the living body than the known rat monoclonal antibody, and suppresses Aggrus-dependent lung metastasis at a lower concentration. An unexpected effect was obtained.
  • the monoclonal antibodies of the present invention recognize different epitopes, and even if resistance mutations that frequently occur in cancer occur, there is a high possibility that they can be overcome by using different antibodies, and have great advantages.
  • the monoclonal antibody of the present invention is a mouse monoclonal antibody, it is necessary to consider species barriers as in the case of a rat antibody in a mouse model transplanted with human cancer (mouse cancer-bearing model) widely used in the development process of anticancer agents.
  • FIG. 14 is a diagram showing the degree of binding of P2-0, MS-1, MS-3, and MS-4 antibodies to recombinant human Aggrus protein using surface plasmon resonance.
  • FIG. 15 shows that P2-0, MS-1, MS-3 and MS-4 antibodies inhibit Aggrus-CLEC-2 interaction.
  • FIG. 16 is a graph showing that P2-0, MS-1, MS-3 and MS-4 antibodies have a platelet aggregation inhibitory effect.
  • FIG. 17 is a diagram showing that MS-1 antibody exerts antitumor activity against human Aggrus-expressing cells.
  • FIG. 18 is a diagram showing that MS-1 antibody inhibits spontaneous metastasis of human Aggrus-expressing cells to the lung.
  • FIG. 19 is a diagram showing that MS-1 and MS-3 antibodies have an effect of suppressing lung metastasis of human Aggrus-expressing cells.
  • the types of dosage forms of the pharmaceutical composition of the present invention include, for example, tablets, powders, pills, powders, granules, fine granules, soft / hard capsules, film coating agents, pellets, tongues as oral preparations Laxatives, pastes, etc., parenteral preparations include injections, suppositories, transdermal preparations, ointments, plasters, liquids for external use, etc. Can be selected.
  • the anti-Aggrus monoclonal antibody as an active ingredient can be contained in the preparation in an amount of 0.1 to 99.9% by weight.
  • Platelet aggregation inhibition test CHO cells and CHO / mock cells are known not to cause platelet aggregation, whereas CHO / Aggrus cells expressing Aggrus caused platelet aggregation.
  • the time from the start of the reaction to the time of the half maximum value was compared. As shown in FIG. 3, it was found that the addition of P2-0 antibody delayed platelet aggregation by Aggrus in a concentration-dependent manner.
  • the recognition of Aggrus expressed in human bladder cancer by the P2-0 antibody was examined by Western blot analysis.
  • the P2-0 antibody recognized Aggrus (lanes 2 to 5) expressed on the surface of various human bladder cancer cell membranes, whereas the commercially available D2-40 antibody (mouse anti-human Aggrus).
  • the monoclonal antibody recognized only the CHO cell line into which the human Aggrus gene was introduced (lane 1), but it was revealed that Aggrus expressed on the surface of the human bladder cancer cell membrane could not be recognized.
  • the CHO cell lines and various human bladder cancer cell lines into which the human Aggrus gene has been introduced were treated under conditions of trypsin treatment (FIG. 9; lanes 7 to 9) or no trypsin treatment (FIG.
  • FIG. 18 shows a graph showing the number of metastatic nodules counted on the upper side, and a photograph of a mouse lung stained with picric acid on the lower side.
  • control antibody mouse IgG2a (Sigma catalog No.

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Abstract

The invention of the application provides a monoclonal antibody or functional fragment thereof that is capable of recognizing epitopes of Aggrus consisting of the amino acid sequence represented by Sequence No. 1, 3, or 4, and a monoclonal antibody or functional fragment thereof that is produced from a hybridoma of deposit No. FERM BP-11446, FERM BP-11447, FERM BP-11448, or FERM BP-11449. The invention provides the hybridoma and further provides an Aggrus-CLEC-2 bond inhibitor and a pharmaceutical composition for the prevention of platelet aggregation or cancer metastasis and for the treatment of tumors or thrombosis that comprises the monoclonal antibody or functional fragment thereof.

Description

マウス抗Aggrusモノクローナル抗体Mouse anti-Aggrus monoclonal antibody
 本願発明は、マウス抗Aggrusモノクローナル抗体に関する。 The present invention relates to a mouse anti-Aggrus monoclonal antibody.
 血小板凝集誘導因子Aggrus(podoplanin、gp44等としても知られる)は、I型膜貫通タンパク質であり、扁平上皮癌、中皮腫、カポジ肉腫、精巣腫瘍及び脳腫瘍といった様々なタイプの癌で発現増加していることが示されている(非特許文献1~9)。Aggrusの過剰発現は予後不良に関係するとの報告があり、癌進行に対するAggrusの重要な関与が示唆されている(非特許文献10、11)。Aggrusの発現が血小板凝集を引き起こし、マウスにおける実験的な、そして自発的な肺転移を促進することが知られている(非特許文献11、12)。血小板凝集を抑制する点突然変異を導入すると、肺転移の形成は減弱するので、Aggrusの血小板凝集誘導活性は転移形成に直接関係していると考えられている(非特許文献11、12)。癌細胞誘導血小板凝集は、大きな癌-血小板凝集を形成し、微小血管系での癌細胞の塞栓形成増大、循環での免疫学的攻撃からの保護に至ると考えられている。最近、血小板上に発現しているC型レクチン様受容体(CLEC-2)が、Aggrusのカウンターパート受容体の一つとして特定された。腫瘍細胞上で発現しているAggrusにCLEC-2が結合すると、血漿成分がなくとも血小板で活性化シグナルが出され、血小板凝集の引き金となることが知られている。相互認識に決定的なAggrus及びCLEC-2のドメインは、すでに知られている(非特許文献13)。 Platelet aggregation-inducing factor Aggrus (also known as podoplanin, gp44, etc.) is a type I transmembrane protein that is upregulated in various types of cancers such as squamous cell carcinoma, mesothelioma, Kaposi's sarcoma, testicular tumor and brain tumor. (Non-Patent Documents 1 to 9). There is a report that overexpression of Aggrus is associated with poor prognosis, suggesting an important involvement of Aggrus in cancer progression (Non-Patent Documents 10 and 11). It is known that the expression of Aggrus causes platelet aggregation and promotes experimental and spontaneous lung metastasis in mice (Non-patent Documents 11 and 12). When a point mutation that suppresses platelet aggregation is introduced, the formation of lung metastasis is attenuated, and thus it is considered that the platelet aggregation-inducing activity of Aggrus is directly related to metastasis formation (Non-patent Documents 11 and 12). Cancer cell-induced platelet aggregation is thought to form large cancer-platelet aggregation, leading to increased embolization of cancer cells in the microvasculature and protection from immunological attack in the circulation. Recently, a C-type lectin-like receptor (CLEC-2) expressed on platelets has been identified as one of the Aggrus counterpart receptors. It is known that when CLEC-2 binds to Aggrus expressed on tumor cells, an activation signal is produced in platelets without plasma components, and triggers platelet aggregation. The domains of Aggrus and CLEC-2 that are critical for mutual recognition are already known (Non-patent Document 13).
 モノクローナル抗体は、細胞表面抗原にしっかりと特異的に結合することができ、標的細胞に免疫学的応答を引き起こすことができる。従って、現在、多くのモノクローナル抗体が癌治療に用いられている。癌治療で用いられるモノクローナル抗体は、中和、抗体依存性細胞傷害活性(antibody-dependent cellular cytotoxicity; ADCC)及び補体依存性細胞傷害活性(complement-dependent cytotoxicity; CDC)、の3つの代表的な作用様式を介して抗癌効果を示す。ベバシズマブやセツキシマブに代表されるように、抗体はリガンド-受容体結合又は受容体多量体化を阻害し、シグナル経路の活性化を中和することができる。癌細胞の増殖はシグナル経路の活性化に依存しているので、その中和により細胞死に至る。他方、リツキシマブやトラスツズマブに代表されるように、抗体はそのFcドメインを介して標的癌細胞に対する免疫応答を誘導することができる。マクロファージ、NK細胞及び好中球等のエフェクター細胞と補体は、癌特異的抗原に結合する抗体のFcドメインを認識し、その結果標的癌細胞を殺す。これらの3つの作用様式は、抗体のアイソタイプやサブクラス、抗原の特徴や認識される部位により規定される。 Monoclonal antibodies can bind specifically and specifically to cell surface antigens and cause an immunological response to target cells. Therefore, many monoclonal antibodies are currently used for cancer treatment. There are three typical monoclonal antibodies used in cancer treatment: neutralization, antibody-dependent cytotoxicity (antibody-dependent cellular cytotoxicity; ADCC) and complement-dependent cytotoxicity (complement-dependent cytotoxicity; CDC). Shows anticancer effects through its mode of action. Antibodies, such as bevacizumab and cetuximab, can inhibit ligand-receptor binding or receptor multimerization and neutralize signal pathway activation. Since the growth of cancer cells depends on the activation of the signal pathway, neutralization thereof leads to cell death. On the other hand, as represented by rituximab and trastuzumab, the antibody can induce an immune response against the target cancer cell via its Fc domain. Effector cells and complements such as macrophages, NK cells, and neutrophils recognize the Fc domain of antibodies that bind to cancer-specific antigens and consequently kill the target cancer cells. These three modes of action are defined by the isotype and subclass of the antibody, the characteristics of the antigen, and the recognized site.
 これまで、Aggrusに対する多くの抗体が確立されてきたが、そのほとんどはAggrus-CLEC-2の相互作用を干渉できないものであった。NZ-1と命名されたラット抗体は、Aggrus-CLEC-2の相互作用および血小板凝集を阻害することができるAggrus抗体として知られているが(非特許文献14)、種のバリアのせいで一般的に用いられるマウスの癌モデルでは正確に調べることができない等の問題点があった。 So far, many antibodies against Aggrus have been established, but most of them were unable to interfere with the Aggrus-CLEC-2 interaction. A rat antibody designated NZ-1 is known as an Aggrus antibody that can inhibit Aggrus-CLEC-2 interaction and platelet aggregation (Non-Patent Document 14), but it is generally due to species barriers. However, the mouse cancer model that is used in general has a problem that it cannot be examined accurately.
 本発明の課題は、Aggrusをターゲットとして癌及び血栓症を処置するための医薬組成物を提供することにある。 An object of the present invention is to provide a pharmaceutical composition for treating cancer and thrombosis with Aggrus as a target.
 本発明者らは、鋭意研究の結果、Aggrus-CLEC-2相互作用及び血小板凝集を阻害することができるモノクローナル抗体を産生するハイブリドーマを樹立した。このハイブリドーマから産生される抗体は、配列番号1(Pro Gly Ala Glu Asp Asp Val Val Thr)、配列番号3(Pro Gly Thr Ser Glu Asp)又は配列番号4(Pro Gly Thr Ser Glu Asp Arg Tyr Lys)により表されるアミノ酸配列からなるAggrusのエピトープを認識すること、Aggrus-CLEC-2の結合を濃度依存的に阻害すること、血小板凝集抑制及び癌の肺転移抑制効果を示すことを見出し、本発明を完成させた。 As a result of diligent research, the present inventors established a hybridoma that produces a monoclonal antibody capable of inhibiting Aggrus-CLEC-2 interaction and platelet aggregation. The antibody produced from this hybridoma is SEQ ID NO: 1 (Pro Gly Ala Glu Asp Asp Val Val Thr), SEQ ID NO: 3 (Pro Gly Thr Ser Glu Asp) or SEQ ID NO: 4 (Pro Gly Thr Ser Glu Asp Arg Tyr Lys) The present invention has been found to recognize the Aggrus epitope consisting of the amino acid sequence represented by the following formula, to inhibit the Aggrus-CLEC-2 binding in a concentration-dependent manner, to suppress platelet aggregation and to suppress lung metastasis of cancer. Was completed.
 すなわち、本発明は、配列番号1、3又は4により表されるアミノ酸配列からなるAggrusのエピトープを認識する、マウスモノクローナル抗体又はその機能的断片からなるフラグメント(1)を提供する。
 また、本発明は、受託番号FERM BP-11446、FERM BP-11447、FERM BP-11448又はFERM BP-11449のハイブリドーマにより産生される、前記(1)記載のモノクローナル抗体又はその機能的断片からなるフラグメント(2)を提供する。
 さらには、本発明は、ヒト化された、前記(1)又は(2)記載のモノクローナル抗体又はその機能的断片からなるフラグメント(3)を提供する。
 本発明は、受託番号FERM BP-11446、FERM BP-11447、FERM BP-11448又はFERM BP-11449のハイブリドーマ(4)を提供する。
 本発明は、前記(1)~(3)のいずれか記載のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、Aggrus-CLEC-2結合阻害剤(5)を提供する。
 本発明は、血小板凝集抑制又は癌転移抑制、あるいは腫瘍又は血栓症の処置のための、前記(1)~(3)のいずれか記載のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、医薬組成物(6)を提供する。
 また、本発明は、血栓症が、脳梗塞又は心筋梗塞である、前記(6)記載の医薬組成物(7)を提供する。
 さらに、本発明は、癌又は腫瘍が、扁平上皮癌、繊維肉腫、中皮腫、カポジ肉腫、精巣腫瘍、脳腫瘍又は膀胱癌である、前記(6)記載の医薬組成物(8)を提供する。
 好ましくは、本発明は、癌又は腫瘍が、扁平上皮癌、中皮腫、精巣腫瘍又は膀胱癌である、前記(8)記載の医薬組成物(9)を提供する。 That is, the present invention provides a fragment (1) comprising a mouse monoclonal antibody or a functional fragment thereof that recognizes an Aggrus epitope comprising the amino acid sequence represented by SEQ ID NO: 1, 3, or 4.
The present invention also relates to a fragment comprising the monoclonal antibody according to the above (1) or a functional fragment thereof produced by a hybridoma of accession number FERM BP-11446, FERM BP-11447, FERM BP-11448 or FERM BP-11449. Provide (2).
Furthermore, the present invention provides a humanized fragment (3) comprising the monoclonal antibody according to (1) or (2) or a functional fragment thereof.
The present invention provides hybridomas (4) with accession numbers FERM BP-11446, FERM BP-11447, FERM BP-11448 or FERM BP-11449.
The present invention provides an Aggrus-CLEC-2 binding inhibitor (5) comprising the monoclonal antibody according to any one of (1) to (3) above or a fragment comprising a functional fragment thereof.
The present invention relates to a medicament comprising a fragment comprising the monoclonal antibody or a functional fragment thereof according to any one of (1) to (3) for inhibiting platelet aggregation, inhibiting cancer metastasis, or treating a tumor or thrombosis. Composition (6) is provided.
The present invention also provides the pharmaceutical composition (7) according to the above (6), wherein the thrombosis is cerebral infarction or myocardial infarction.
Furthermore, the present invention provides the pharmaceutical composition (8) according to (6) above, wherein the cancer or tumor is squamous cell carcinoma, fibrosarcoma, mesothelioma, Kaposi sarcoma, testicular tumor, brain tumor or bladder cancer. .
Preferably, the present invention provides the pharmaceutical composition (9) described in (8) above, wherein the cancer or tumor is squamous cell carcinoma, mesothelioma, testicular tumor or bladder cancer.
 本発明者らが樹立したハイブリドーマから産生されるP2-0、MS-1、MS-3、MS-4と命名されたマウスモノクローナル抗体は、in vivo及びin vitroで分析したところ、配列番号1、3又は4により表されるアミノ酸配列からなるAggrusのエピトープを認識し、Aggrus-CLEC-2の結合を濃度依存的に阻害することが分かった。また、本願発明のモノクローナル抗体は、血小板凝集抑制効果や癌の肺転移抑制効果も示した。本願発明のモノクローナル抗体のヒト化抗体(ヒト型キメラ抗体)は、Aggrus低発現細胞にも癌転移抑制効果を示した。本願発明のモノクローナル抗体は、既に知られているラットのモノクローナル抗体よりも、生体で発現しているネイティブなAggrusに対する反応性が異なっており、Aggrus依存的な肺転移をより低濃度で抑制するという、予測し得ない効果が得られた。また、本願発明のモノクローナル抗体は各々異なるエピトープを認識しており、癌で頻発する耐性変異などが生じた場合でも別の抗体を用いれば克服できる可能性が高く、大きな利点を有している。さらに本願発明のモノクローナル抗体はマウスモノクローナル抗体であるため、抗癌剤の開発過程で汎用されるヒト癌を移植したマウスモデル(マウス担癌モデル)において、ラット抗体のように種のバリアを考慮する必要が無い。一般に、CDRをマウス抗体のFcドメインに結合させることにより、マウスキメラ抗体をラット抗体から作製することもできるとはいえ、そのマウスキメラ抗体の産生にはCHO細胞などの抗体産生細胞にキメラ抗体発現ベクターを遺伝子導入して産生させることが必要であり、マウスキメラ抗体の大量精製にはマウス抗体をマウス腹水で産生させる場合と比べて経済的ではなく、実用に適さない。よって、本願発明のマウスモノクローナル抗体は、例えばヒト癌のマウス担癌モデルを用いた医薬組成物の開発に格別に利便性を有する。 The mouse monoclonal antibodies designated P2-0, MS-1, MS-3, and MS-4 produced from the hybridoma established by the present inventors were analyzed in vivo and in vitro. It was found that the epitope of Aggrus consisting of the amino acid sequence represented by 3 or 4 was recognized, and binding of Aggrus-CLEC-2 was inhibited in a concentration-dependent manner. In addition, the monoclonal antibody of the present invention also showed an effect of suppressing platelet aggregation and an effect of suppressing lung metastasis of cancer. The humanized antibody (human chimeric antibody) of the monoclonal antibody of the present invention showed an effect of suppressing cancer metastasis even in cells with low expression of Aggrus. The monoclonal antibody of the present invention is different in reactivity to native Aggrus expressed in the living body than the known rat monoclonal antibody, and suppresses Aggrus-dependent lung metastasis at a lower concentration. An unexpected effect was obtained. In addition, the monoclonal antibodies of the present invention recognize different epitopes, and even if resistance mutations that frequently occur in cancer occur, there is a high possibility that they can be overcome by using different antibodies, and have great advantages. Furthermore, since the monoclonal antibody of the present invention is a mouse monoclonal antibody, it is necessary to consider species barriers as in the case of a rat antibody in a mouse model transplanted with human cancer (mouse cancer-bearing model) widely used in the development process of anticancer agents. No. In general, a mouse chimeric antibody can be produced from a rat antibody by binding a CDR to the Fc domain of a mouse antibody, but the chimeric antibody is expressed in antibody-producing cells such as CHO cells for the production of the mouse chimeric antibody. It is necessary to introduce a vector into a gene and produce it, and mass purification of a mouse chimeric antibody is less economical than the case of producing a mouse antibody in mouse ascites and is not suitable for practical use. Therefore, the mouse monoclonal antibody of the present invention has particular convenience in developing a pharmaceutical composition using, for example, a mouse tumor bearing model of human cancer.
図1は、P2-0抗体の合成ペプチドを用いた認識エピトープの絞り込みを示す図である。FIG. 1 is a diagram showing the narrowing of recognition epitopes using a synthetic peptide of the P2-0 antibody. 図2は、P2-0抗体が、濃度依存的にAggrus-CLEC-2相互作用を阻害することを示す図である。FIG. 2 shows that the P2-0 antibody inhibits the Aggrus-CLEC-2 interaction in a concentration-dependent manner. 図3は、P2-0抗体が、血小板凝集抑制効果を有することを示す図である。FIG. 3 is a graph showing that the P2-0 antibody has a platelet aggregation inhibitory effect. 図4は、P2-0抗体が、癌の肺転移抑制効果を有することを示す図である。FIG. 4 is a graph showing that the P2-0 antibody has an effect of suppressing lung metastasis of cancer. 図5は、ヒト化P2-0抗体(ヒト型キメラP2-0抗体)が、血小板凝集抑制効果を有することを示す図である。FIG. 5 is a graph showing that humanized P2-0 antibody (human chimeric P2-0 antibody) has a platelet aggregation inhibitory effect. 図6は、ヒト化P2-0抗体(ヒト型キメラP2-0抗体)が、癌の肺転移抑制効果を有することを示す図である。FIG. 6 shows that humanized P2-0 antibody (human chimeric P2-0 antibody) has an effect of suppressing lung metastasis of cancer. 図7は、ヒト化P2-0抗体(ヒト型キメラP2-0抗体)が、Aggrus低発現細胞(HT1080細胞)にも肺転移抑制効果を有することを示す図である。FIG. 7 is a view showing that humanized P2-0 antibody (human chimeric P2-0 antibody) also has an effect of suppressing lung metastasis in Aggrus low-expressing cells (HT1080 cells). 図8は、P2-0抗体が、ヒト膀胱癌細胞膜表面に発現しているAggrusを認識することを示すウェスタンブロット分析の図である。FIG. 8 is a Western blot analysis showing that the P2-0 antibody recognizes Aggrus expressed on the surface of human bladder cancer cell membrane. 図9は、NZ-1抗体とP2-0抗体とのAggrus認識能の違いを示すウェスタンブロット分析の図である。FIG. 9 is a Western blot analysis showing the difference in Aggrus recognition ability between the NZ-1 antibody and the P2-0 antibody. 図10Aは、NZ-1抗体(図10A)とP2-0抗体(図10B)とのAggrus認識能の違いを示すFACS法におけるNZ-1抗体の解析結果の図である。FIG. 10A is a diagram of the results of analysis of the NZ-1 antibody in the FACS method showing the difference in the ability to recognize Aggrus between the NZ-1 antibody (FIG. 10A) and the P2-0 antibody (FIG. 10B). 図10Bは、NZ-1抗体(図10A)とP2-0抗体(図10B)とのAggrus認識能の違いを示すFACS法におけるP2-0抗体の解析結果の図である。FIG. 10B is a diagram showing the results of analysis of the P2-0 antibody in the FACS method, showing the difference in Aggrus recognition ability between the NZ-1 antibody (FIG. 10A) and the P2-0 antibody (FIG. 10B). 図11は、NZ-1抗体とP2-0抗体との癌の肺転移抑制効果の違いを示す図である。FIG. 11 is a graph showing the difference in pulmonary metastasis inhibitory effect of NZ-1 antibody and P2-0 antibody on cancer. 図12は、MS-1、MS-3およびMS-4抗体がヒトAggrusを認識することを、ヒトAggrus遺伝子を導入したCHO細胞株を用いたフローサイトメトリー解析により確認した図である。FIG. 12 shows that the MS-1, MS-3, and MS-4 antibodies recognize human Aggrus by flow cytometry analysis using a CHO cell line into which the human Aggrus gene has been introduced. 図13は、アラニン変異型Aggrusタンパク質を用いたP2-0、MS-1、MS-3およびMS-4抗体の認識エピトープの絞り込みを示す図である。FIG. 13 is a diagram showing the narrowing of recognition epitopes of P2-0, MS-1, MS-3, and MS-4 antibodies using an alanine mutant Aggrus protein. 図14は、表面プラズモン共鳴を用いた組換えヒトAggrusタンパク質に対するP2-0、MS-1、MS-3およびMS-4抗体の結合度を測定した図である。FIG. 14 is a diagram showing the degree of binding of P2-0, MS-1, MS-3, and MS-4 antibodies to recombinant human Aggrus protein using surface plasmon resonance. 図15は、P2-0、MS-1、MS-3およびMS-4抗体がAggrus-CLEC-2相互作用を阻害することを示す図である。FIG. 15 shows that P2-0, MS-1, MS-3 and MS-4 antibodies inhibit Aggrus-CLEC-2 interaction. 図16は、P2-0、MS-1、MS-3およびMS-4抗体が血小板凝集抑制効果を有することを示す図である。FIG. 16 is a graph showing that P2-0, MS-1, MS-3 and MS-4 antibodies have a platelet aggregation inhibitory effect. 図17は、MS-1抗体がヒトAggrus発現細胞に対して抗腫瘍活性を発揮することを示す図である。FIG. 17 is a diagram showing that MS-1 antibody exerts antitumor activity against human Aggrus-expressing cells. 図18は、MS-1抗体がヒトAggrus発現細胞の肺への自然転移を阻害することを示す図である。FIG. 18 is a diagram showing that MS-1 antibody inhibits spontaneous metastasis of human Aggrus-expressing cells to the lung. 図19は、MS-1およびMS-3抗体がヒトAggrus発現細胞の肺転移抑制効果を有することを示す図である。FIG. 19 is a diagram showing that MS-1 and MS-3 antibodies have an effect of suppressing lung metastasis of human Aggrus-expressing cells.
 Aggrusは、gp44、podoplanin等としても知られている。 Aggrus is also known as gp44, podoplanin, etc.
 「抗Aggrusモノクローナル抗体」は、Aggrusに特異的に結合するモノクローナル抗体または誘導体をいい、元の抗体と実質的に同じ抗原特異性を示す当該抗体の断片(本明細書中、「機能的断片」と呼ぶ)をも含むものとする。抗体の機能的断片には、Fab、Fab'、F(ab')2、単鎖抗体(scFv)、ジスルフィド安定化V領域断片(dsFv)、もしくはCDRを含むペプチドなどの抗体の機能的断片などが含まれる。本発明における抗体は、以下に詳述するように、動物、好ましくはマウスを免疫し、適切な細胞との融合によるハイブリドーマの作製のため脾臓細胞を回収することを含む、従来の方法により作製することができる。 “Anti-Aggrus monoclonal antibody” refers to a monoclonal antibody or derivative that specifically binds to Aggrus, and a fragment of the antibody that exhibits substantially the same antigen specificity as the original antibody (referred to herein as a “functional fragment”). Also called). Functional fragments of antibodies include Fab, Fab ′, F (ab ′) 2 , single chain antibodies (scFv), disulfide stabilized V region fragments (dsFv), or antibody functional fragments such as CDR-containing peptides, etc. Is included. The antibodies in the present invention are produced by conventional methods, including immunizing an animal, preferably a mouse, and collecting spleen cells for hybridoma production by fusion with appropriate cells, as described in detail below. be able to.
 Aggrusに対するマウスモノクローナル抗体の好適な例としては、独立行政法人 産業技術総合研究所 特許生物寄託センター(IPOD;日本国〒305-8566 茨城県つくば市東1丁目1番地1中央第6)に受託番号FERM BP-11446として2011年2月18日付で寄託されたハイブリドーマ、並びに受託番号FERM BP-11447、FERM BP-11448及びFERM BP-11449として前記IPODに2011年12月28日付で寄託されたハイブリドーマが産生するモノクローナル抗体が挙げられる。また、これと同等の結合特性を有する他の抗体も本発明の抗Aggrusモノクローナル抗体として好ましい。 As a suitable example of a mouse monoclonal antibody against Aggrus, the accession number FERM can be found at the National Institute of Advanced Industrial Science and Technology, Patent Biological Depositary Center (IPOD; 1st, 1st, 1-chome, 1-chome, Tsukuba, Japan 305-8566). Hybridomas deposited as BP-11446 on February 18, 2011, and hybridomas deposited with the IPOD as deposit numbers FERM BP-11447, FERM BP-11448 and FERM BP-11449 on December 28, 2011 And monoclonal antibodies. Other antibodies having binding properties equivalent to this are also preferable as the anti-Aggrus monoclonal antibody of the present invention.
 ヒト以外の動物の抗体を、遺伝子組換え技術を利用してヒト型キメラ抗体あるいはヒト型CDR移植抗体などとしたヒト化抗体もまた、本発明において有利に使用することができる。ヒト型キメラ抗体とは、抗体の可変領域(以下、V領域と表記する)がヒト以外の動物の抗体で、定常領域(以下、C領域と表記する)がヒト抗体である抗体であり(Morrison S.L. et al.、Proc Natl Acad Sci USA.81(21),6851-6855,1984)、ヒト型CDR移植抗体とは、ヒト以外の動物の抗体のV領域中のCDRのアミノ酸配列をヒト抗体の適切な位置に移植した抗体である(Jones P.T. et al.、Nature,321(6069),522-525,1986)。ヒト化抗体は、ヒトに投与した場合、ヒト以外の動物の抗体に比べ、副作用が少なく、その治療効果が長期間持続する。また、ヒト化抗体は、遺伝子組換え技術を利用して様々な形態の分子として作製することができる。 A humanized antibody obtained by using a non-human animal antibody as a human chimeric antibody or a human CDR-grafted antibody using a gene recombination technique can also be advantageously used in the present invention. A human chimeric antibody is an antibody in which the variable region of an antibody (hereinafter referred to as V region) is an antibody of a non-human animal, and the constant region (hereinafter referred to as C region) is a human antibody (Morrison SL et al., Proc Natl Acad Sci USA.81 (21), 6851-6855, 1984), human CDR-grafted antibody refers to the CDR amino acid sequence in the V region of an antibody from a non-human animal. It is an antibody transplanted at an appropriate position (Jones PT et al., Nature, 321 (6069), 522-525, 1986). When administered to humans, humanized antibodies have fewer side effects than antibodies from non-human animals, and their therapeutic effects last for a long time. In addition, humanized antibodies can be prepared as molecules of various forms using gene recombination techniques.
 本発明は、別の態様において、本願発明のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、Aggrus-CLEC-2結合阻害剤、及び血小板凝集抑制又は癌転移抑制、あるいは腫瘍又は血栓症の処置のための、本願発明のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、医薬組成物を提供する。血栓症は、好ましくは脳梗塞又は心筋梗塞である。癌又は腫瘍は、好ましくは扁平上皮癌、繊維肉腫、中皮腫、カポジ肉腫、精巣腫瘍、脳腫瘍又は膀胱癌である。なお、本願明細書中、用語「癌」と「腫瘍」とは同じ意味を有する用語として使用される。 In another aspect, the present invention relates to an Aggrus-CLEC-2 binding inhibitor comprising the monoclonal antibody of the present invention or a fragment consisting of a functional fragment thereof, and platelet aggregation suppression or cancer metastasis suppression, or treatment of tumor or thrombosis A pharmaceutical composition comprising a fragment consisting of the monoclonal antibody of the present invention or a functional fragment thereof is provided. The thrombosis is preferably cerebral infarction or myocardial infarction. The cancer or tumor is preferably squamous cell carcinoma, fibrosarcoma, mesothelioma, Kaposi sarcoma, testicular tumor, brain tumor or bladder cancer. In the present specification, the terms “cancer” and “tumor” are used as terms having the same meaning.
 本発明の医薬組成物の剤型の種類としては、例えば、経口剤として錠剤、粉末剤、丸剤、散剤、顆粒剤、細粒剤、軟・硬カプセル剤、フィルムコーティング剤、ペレット剤、舌下剤、ペースト剤等、非経口剤として注射剤、坐剤、経皮剤、軟膏剤、硬膏剤、外用液剤等が挙げられ、当業者においては投与経路や投与対象等に応じた最適の剤型を選ぶことができる。有効成分としての抗Aggrusモノクローナル抗体は、製剤中0.1から99.9重量%含有することができる。 The types of dosage forms of the pharmaceutical composition of the present invention include, for example, tablets, powders, pills, powders, granules, fine granules, soft / hard capsules, film coating agents, pellets, tongues as oral preparations Laxatives, pastes, etc., parenteral preparations include injections, suppositories, transdermal preparations, ointments, plasters, liquids for external use, etc. Can be selected. The anti-Aggrus monoclonal antibody as an active ingredient can be contained in the preparation in an amount of 0.1 to 99.9% by weight.
 本発明の薬剤の有効成分の投与量は、投与対象、対象臓器、症状、投与方法などにより差はあるが、経口投与の場合、一般的に例えば、患者(60kgとして)に対して一日につき約0.1μg~1000mg、好ましくは約1.0μg~100mg、より好ましくは約1.0mg~50mgである。非経口的に投与する場合は、その一回投与量は投与対象、対象臓器、症状、投与方法などによっても異なるが、例えば、注射剤の形では通常例えば、患者(60kgに対して)、一日につき約0.01から30mg程度、好ましくは約0.1から20mg程度、より好ましくは約0.1~10mg程度を静脈注射により投与するのが好都合である。しかしながら、最終的には、剤型の種類、投与方法、患者の年齢や体重、患者の症状等を考慮して、医師または獣医師の判断により適宜決定することができる。
 以下に実施例を挙げて、本願発明を詳細に説明する。 The dose of the active ingredient of the drug of the present invention varies depending on the administration subject, target organ, symptom, administration method, etc., but in the case of oral administration, for example, generally for a patient (as 60 kg) per day The amount is about 0.1 μg to 1000 mg, preferably about 1.0 μg to 100 mg, more preferably about 1.0 mg to 50 mg. When administered parenterally, the single dose varies depending on the administration subject, target organ, symptom, administration method, etc. For example, in the form of an injection, for example, a patient (for 60 kg), It is convenient to administer about 0.01 to 30 mg per day, preferably about 0.1 to 20 mg, more preferably about 0.1 to 10 mg by intravenous injection. However, the final decision can be made as appropriate based on the judgment of a doctor or veterinarian in consideration of the type of dosage form, administration method, patient age and weight, patient symptoms, and the like.
Hereinafter, the present invention will be described in detail with reference to examples.
マウス抗ヒトAggrusモノクローナル抗体産生ハイブリドーマの作製
免疫原
 ヒトAggrus cDNAのTT679部位(位置38~51の14個のアミノ酸(配列番号2:Glu Gly Gly Val Ala Met Pro Gly Ala Glu Asp Asp Val Val)をクローニングし、pGEX-6P-3ベクター(GE Healthcare、英国バッキンガムシャー州)に8回反復してつないだ(TT679-repeat)。このベクターで大腸菌BL21(Invitrogen、カリフォルニア州カールズバッド)を形質転換し、そしてGSTタグ付け組換えタンパク質をGlutathione Sepharose(GE Healthcare)により精製した。 Production of mouse anti-human Aggrus monoclonal antibody-producing hybridoma
The TT679 site (SEQ ID NO: 2: Glu Gly Gly Val Ala Met Pro Gly Ala Glu Asp Asp Val Val) of the immunogenic human Aggrus cDNA was cloned into pGEX-6P-3 vector (GE (TT679-repeat) E. coli BL21 (Invitrogen, Carlsbad, Calif.) Was transformed with this vector and the GST-tagged recombinant protein was transferred to Glutathione Sepharose (GE Purified by Healthcare).
感作
 6週齢の雌性BALB/cマウス(日本チャールズリバー株式会社から購入し、常法に従って飼育)に、Freund's complete adjuvant(Difco Laboratories、ミシガン州デトロイト)を用いて上記で得られた免疫原を頸部皮下投与した。隔週での腹腔内投与により、追加免疫を行った。 The immunogen obtained above using Freund's complete adjuvant (Difco Laboratories, Detroit, Mich.) On 6-week-old female BALB / c mice (purchased from Charles River Japan, Inc. The neck was administered subcutaneously. Booster immunization was performed by intraperitoneal administration every other week.
ハイブリドーマ樹立
 常法に従って、脾臓細胞を採取し、ポリエチレングリコール4000(Merck、ニュージャージー州)を用いてマウスミエローマ細胞P3U1と融合させた。ヒポキサンチン、アミノプテリン及びチミジンを含むRPMI 1640培地(Sigma)で増殖させて、ハイブリドーマを選択した。その結果、15クローンのハイブリドーマが樹立された。 Spleen cells were collected and fused with mouse myeloma cells P3U1 using polyethylene glycol 4000 (Merck, NJ) according to the conventional method of hybridoma establishment . Hybridomas were selected by growing in RPMI 1640 medium (Sigma) containing hypoxanthine, aminopterin and thymidine. As a result, 15 clone hybridomas were established.
マウス抗ヒトAggrusモノクローナル抗体の分析
ウェスタンブロットによる検証
 上記で得られたハイブリドーマから得られる抗体のうち、P2-0という抗体を産生するハイブリドーマを、2011年2月18日に、独立行政法人 産業技術総合研究所 特許生物寄託センターに寄託し、受託番号FERM BP-11446を付された(受託番号FERM P-22069と同一)。P2-0抗体は、フローサイトメトリー及びウェスタンブロット分析により、ヒトAggrusを認識することが示された。さらに、配列番号2で示されるアミノ酸配列が欠失したAggrus変異体を作製してウェスタンブロット分析を行ったところ、P2-0抗体はこれを認識できなかった。 Analysis of mouse anti-human Aggrus monoclonal antibody
Verification by Western blot Of the antibodies obtained from the hybridoma obtained above, a hybridoma producing the antibody P2-0 was deposited on February 18, 2011 at the National Institute of Advanced Industrial Science and Technology, Patent Organism Depositary. Accession No. FERM BP-11446 (same as Accession No. FERM P-22069). The P2-0 antibody was shown to recognize human Aggrus by flow cytometry and Western blot analysis. Further, when an Aggrus mutant lacking the amino acid sequence shown in SEQ ID NO: 2 was prepared and subjected to Western blot analysis, the P2-0 antibody could not recognize this.
エピトープの探索
 図1に示されるように、様々なペプチドを化学合成し、それらに対するP2-0抗体の反応性をELISA法にて検討した。その結果、位置44~52のアミノ酸配列(配列番号1)を有するペプチドに対して高い反応性が示された。 As shown in FIG. 1, various peptides were chemically synthesized, and the reactivity of the P2-0 antibody to them was examined by ELISA. As a result, high reactivity was shown with respect to the peptide having the amino acid sequence at positions 44 to 52 (SEQ ID NO: 1).
Aggrus-CLEC-2結合阻害試験
 哺乳動物細胞から精製した組換えAggrusタンパク質及びCLEC-2タンパク質を用いて、Aggrus-CLEC-2相互作用をELISA法により検出した。Aggrus抗体の存在下での相互作用への影響を調べた。図2に示されるように、P2-0抗体は、濃度依存的にAggrus-CLEC-2相互作用を阻害することが見出された。 Aggrus-CLEC-2 binding inhibition test Aggrus-CLEC-2 interaction was detected by ELISA using recombinant Aggrus protein and CLEC-2 protein purified from mammalian cells. The influence on the interaction in the presence of Aggrus antibody was examined. As shown in FIG. 2, the P2-0 antibody was found to inhibit Aggrus-CLEC-2 interaction in a concentration-dependent manner.
血小板凝集抑制試験
 CHO細胞及びCHO/mock細胞は、血小板凝集を引き起こせないことが知られているのに対し、Aggrusを発現したCHO/Aggrus細胞は血小板凝集を引き起こした。光線透過率のモニタリングによるin vitro血小板凝集分析において、反応開始時点から最大の半分の値の時点までの時間を比較した。図3に示されるように、P2-0抗体の添加により、Aggrusによる血小板凝集は濃度依存的に遅延されることが見出された。 Platelet aggregation inhibition test CHO cells and CHO / mock cells are known not to cause platelet aggregation, whereas CHO / Aggrus cells expressing Aggrus caused platelet aggregation. In the in vitro platelet aggregation analysis by monitoring light transmittance, the time from the start of the reaction to the time of the half maximum value was compared. As shown in FIG. 3, it was found that the addition of P2-0 antibody delayed platelet aggregation by Aggrus in a concentration-dependent manner.
肺転移抑制試験
 静脈注射後、ヒトAggrus遺伝子を導入したCHO細胞株のin vivoにおける実験的肺転移に対する抗体の影響を検討した。CHO細胞は、Aggrusの強制発現により転移性となることが知られている。図4に示されるように、P2-0抗体は、0.1μg/匹といった非常に少量でも非常に強い肺転移抑制効果を示すことが明らかとなり、P2-0抗体はAggrus中和活性だけでなく、Aggrus依存的な血行性転移を阻害することも示された。 Lung metastasis suppression test After intravenous injection, the effect of antibodies on experimental lung metastasis in vivo of the CHO cell line introduced with the human Aggrus gene was examined. It is known that CHO cells become metastatic by forced expression of Aggrus. As shown in FIG. 4, it is clear that the P2-0 antibody exhibits a very strong lung metastasis inhibitory effect even at a very small amount of 0.1 μg / animal. It has also been shown to inhibit Aggrus-dependent hematogenous metastasis.
ヒト化抗体の作製と検証
 実用可能とするために、P2-0抗体のAggrus認識可変領域をクローニングし、定法に従ってヒトIgGの定常領域に組み込んだヒト化P2-0抗体(ヒト型キメラP2-0抗体)を作製した。また、このヒト化P2-0抗体は、サルAggrusを認識することを確認した。さらに、このヒト化P2-0抗体は、元のP2-0抗体と同様に血小板凝集阻害活性(図5)及び癌の転移抑制効果(図6)を示すことも確認した。このヒト化P2-0抗体は、図7に示されるように、Aggrus低発現細胞(HT1080細胞)にも癌転移抑制効果を示した。 Preparation and verification of humanized antibody In order to make it practical, the humanized P2-0 antibody (human chimeric P2-0) in which the Aggrus recognition variable region of the P2-0 antibody was cloned and incorporated into the constant region of human IgG according to a conventional method Antibody). It was also confirmed that this humanized P2-0 antibody recognizes monkey Aggrus. Furthermore, it was also confirmed that this humanized P2-0 antibody showed platelet aggregation inhibitory activity (FIG. 5) and cancer metastasis inhibitory effect (FIG. 6) in the same manner as the original P2-0 antibody. As shown in FIG. 7, this humanized P2-0 antibody also showed a cancer metastasis inhibitory effect on Aggrus low-expressing cells (HT1080 cells).
Aggrus関連癌の探索とラット抗Aggrus抗体(NZ-1抗体)との比較
 本発明者らはさらに、Aggrusが膀胱癌でも高頻度に発現亢進していることを、膀胱癌の臨床サンプルより得られたcDNA(OriGene社より市販されているTissueScan cDNA Panel)をテンプレートとしたreal-time PCR法により見いだした。 Search for Aggrus-related cancer and comparison with rat anti-Aggrus antibody (NZ-1 antibody) The present inventors further obtained from clinical samples of bladder cancer that Aggrus is highly upregulated in bladder cancer. It was found by real-time PCR using a cDNA (TissueScan cDNA Panel commercially available from OriGene) as a template.
 そこで、ウェスタンブロット分析により、ヒト膀胱癌に発現しているAggrusのP2-0抗体による認識を調べた。図8に示されるように、P2-0抗体は、各種ヒト膀胱癌細胞膜表面に発現しているAggrus(レーン2~5)を認識したのに対し、市販のD2-40抗体(マウス抗ヒトAggrusモノクローナル抗体)は、ヒトAggrus遺伝子を導入したCHO細胞株のみ(レーン1)を認識したが、ヒト膀胱癌細胞膜表面に発現しているAggrusを認識できないことが明らかとなった。さらに、ヒトAggrus遺伝子を導入したCHO細胞株及び各種ヒト膀胱癌細胞株を、タンパク質分解酵素であるトリプシン処理の条件下(図9;レーン7~9)あるいはトリプシン無処理の条件下(図9;レーン12~15)で回収し、その細胞溶解液をSDS-PAGEし、P2-0抗体、NZ-1抗体とタンパク質泳動量が揃っていることを確認するためのアクチン抗体でウェスタンブロット分析を行った。その結果、図9に示されるように、P2-0抗体はヒト膀胱癌細胞膜表面に発現しているAggrusタンパク質を認識したが、NZ-1抗体はヒトAggrusを導入したCHO細胞に発現しているAggrusしか認識できず(図9;レーン6)、ヒト膀胱癌細胞膜表面に発現している野生型Aggrusを認識することができないことが明らかとなった。 Therefore, the recognition of Aggrus expressed in human bladder cancer by the P2-0 antibody was examined by Western blot analysis. As shown in FIG. 8, the P2-0 antibody recognized Aggrus (lanes 2 to 5) expressed on the surface of various human bladder cancer cell membranes, whereas the commercially available D2-40 antibody (mouse anti-human Aggrus). The monoclonal antibody) recognized only the CHO cell line into which the human Aggrus gene was introduced (lane 1), but it was revealed that Aggrus expressed on the surface of the human bladder cancer cell membrane could not be recognized. Furthermore, the CHO cell lines and various human bladder cancer cell lines into which the human Aggrus gene has been introduced were treated under conditions of trypsin treatment (FIG. 9; lanes 7 to 9) or no trypsin treatment (FIG. 9; Lanes 12 to 15), and the cell lysate is subjected to SDS-PAGE, and Western blot analysis is performed with an actin antibody to confirm that P2-0 antibody and NZ-1 antibody and the protein migration amount are aligned. It was. As a result, as shown in FIG. 9, the P2-0 antibody recognized the Aggrus protein expressed on the surface of the human bladder cancer cell membrane, while the NZ-1 antibody was expressed in CHO cells into which human Aggrus was introduced. Only Aggrus could be recognized (FIG. 9; lane 6), indicating that wild-type Aggrus expressed on the surface of human bladder cancer cell membrane could not be recognized.
 本検討により、P2-0抗体はこれまでに知られていた抗ヒトAggrus抗体(NZ-1を含む)と比較して、生体で発現しているネイティブAggrusに対する反応性が強いことが実証され、P2-0抗体は多種類の癌で発現しているAggrusを認識できる抗体であることが示唆された。従って、P2-0抗体はAggrusをターゲットとした使用において、より優れた効果を有することが示唆された。 This study demonstrates that the P2-0 antibody is more reactive to native Aggrus expressed in the living body than the anti-human Aggrus antibody (including NZ-1) known so far, It was suggested that the P2-0 antibody is an antibody that can recognize Aggrus expressed in various types of cancer. Therefore, it was suggested that the P2-0 antibody has a better effect in the use targeting Aggrus.
 さらに、FACS法により、上記ウェスタンブロット分析の結果を再現した。具体的には、ヒト膀胱癌細胞株T24をタンパク質分解酵素であるトリプシンを含まないEDTAのみで細胞回収し、その細胞に対してそれぞれNZ-1抗体又はそのコントロール抗体であるラット抗体を4℃で1時間反応させた。過剰な抗体をPBSで洗浄した後、2次抗体としてAlexa488標識された抗ラットIgG抗体を4℃で1時間反応させた。過剰な抗体をPBSで洗浄した後、Beckman Coulter社のCytomics FC500フローサイトメーターで解析した。結果を、図10Aに示す。 Furthermore, the result of the Western blot analysis was reproduced by FACS method. Specifically, a human bladder cancer cell line T24 was recovered with only EDTA not containing trypsin, which is a proteolytic enzyme, and NZ-1 antibody or a rat antibody, which is a control antibody, was applied to the cells at 4 ° C. The reaction was carried out for 1 hour. After the excess antibody was washed with PBS, Alexa488-labeled anti-rat IgG antibody as a secondary antibody was reacted at 4 ° C. for 1 hour. Excess antibody was washed with PBS and analyzed with a Cytomics FC500 flow cytometer from Beckman Coulter. The results are shown in FIG. 10A.
 他方、上記回収したヒト膀胱癌細胞株T24に対してそれぞれP2-0抗体又はそのコントロール抗体であるマウス抗体を4℃で1時間反応させた。過剰な抗体をPBSで洗浄した後、2次抗体としてAlexa488標識された抗マウスIgG抗体を4℃で1時間反応させた。過剰な抗体をPBSで洗浄した後、同様にフリーサイトメーターで解析した。結果を、図10Bに示す。図10A及びBに示されるように、NZ-1抗体はヒト膀胱癌細胞株T24に発現しているAggrusを認識しなかったが、P2-0抗体は認識していた。 On the other hand, the collected human bladder cancer cell line T24 was reacted with a P2-0 antibody or a mouse antibody as its control antibody at 4 ° C. for 1 hour. After the excess antibody was washed with PBS, Alexa488-labeled anti-mouse IgG antibody as a secondary antibody was reacted at 4 ° C. for 1 hour. Excess antibody was washed with PBS and similarly analyzed with a free cytometer. The results are shown in FIG. 10B. As shown in FIGS. 10A and B, the NZ-1 antibody did not recognize Aggrus expressed in the human bladder cancer cell line T24, but recognized the P2-0 antibody.
 ヒトAggrus遺伝子を導入したCHO細胞株のin vivoにおける実験的肺転移に対するP2-0抗体とNZ-1抗体の作用を比較した。図11に示されるように、P2-0抗体は、マウス1匹当たり0.01μg、0.001μgといった非常に少量でもコントロール抗体投与群と比較して有意に肺転移抑制効果を示すが、NZ-1抗体は、0.1μg/匹では有意な転移抑制効果を示すが、0.01μg/匹、0.001μg/匹といった少量ではコントロール抗体と比較して有意な抑制効果を示せないことが明らかとなった。よって、P2-0抗体はNZ-1抗体と比較して強い血行性転移阻害活性を持つことが明らかとなった。従って、P2-0抗体は、Aggrus認識およびAggrus機能抑制において優れた効果を有する抗体であり、実験的・臨床的使用において有利であることが見出された。 The effects of P2-0 antibody and NZ-1 antibody on experimental lung metastasis in vivo of CHO cell lines into which the human Aggrus gene was introduced were compared. As shown in FIG. 11, the P2-0 antibody shows a significant effect of suppressing lung metastasis compared to the control antibody administration group even at a very small amount of 0.01 μg and 0.001 μg per mouse. It is apparent that 1 antibody shows a significant metastasis inhibitory effect at 0.1 μg / animal but does not show a significant inhibitory effect compared to the control antibody at small amounts of 0.01 μg / animal and 0.001 μg / animal. became. Therefore, it was revealed that the P2-0 antibody has stronger hematogenous metastasis inhibitory activity than the NZ-1 antibody. Therefore, the P2-0 antibody is an antibody having an excellent effect in Aggrus recognition and suppression of Aggrus function, and was found to be advantageous in experimental and clinical use.
マウス抗ヒトAggrusモノクローナル抗体産生ハイブリドーマの作製
免疫原
 ヒトAggrus cDNAのPP4262部位(位置42~62の21個のアミノ酸(配列番号5:Ala Met Pro Gly Ala Glu Asp Asp Val Val Thr Pro Gly Thr Ser Glu Asp Arg Tyr Lys Ser))を18回繰り返したものをpGEX-6P3ベクター(GE Healthcare)にクローニングした。このベクターで大腸菌BL21(Invitrogen)を形質転換し、GSTタグ融合組み換えタンパク質をGlutathione Sepharose(GE Healthcare)により精製した。 Production of mouse anti-human Aggrus monoclonal antibody-producing hybridoma
PP4262 site (21 amino acids at positions 42 to 62 (SEQ ID NO: 5: Ala Met Pro Gly Ala Glu Asp Asp Val Val Thr Pro Gly Thr Ser Glu Asp Arg Tyr Lys Ser)) of the immunogen human Aggrus cDNA is repeated 18 times. Was cloned into the pGEX-6P3 vector (GE Healthcare). Escherichia coli BL21 (Invitrogen) was transformed with this vector, and the GST-tagged recombinant protein was purified by Glutathione Sepharose (GE Healthcare).
感作
 6週齢の雌性BALB/cマウス(日本チャールズリバー株式会社から購入し、常法に従って飼育)に、TiterMax Gold(TiterMax USA, Inc.)を用いて上記で得られた免疫原を頸部皮下投与した。隔週での腹腔内投与により、追加免疫を行った。 Sensitized 6-week-old female BALB / c mice (purchased from Japan Charles River Co., Ltd. and reared according to conventional methods) were subjected to the immunogen obtained above using TiterMax Gold (TiterMax USA, Inc.). It was administered subcutaneously. Booster immunization was performed by intraperitoneal administration every other week.
ハイブリドーマ樹立
 常法に従って脾臓細胞を採取し、ポリエチレングリコール4000(Merck)を用いてマウスミエローマ細胞P3U1と融合させた。ヒポキサンチン、アミノプテリンおよびチミジンを含むエス・クロン クローニングメディウム(エーディア株式会社)で増殖させて、ハイブリドーマを選択した。その結果、複数個のハイブリドーマが樹立された。 Spleen cells were collected according to the conventional method of hybridoma establishment, and fused with mouse myeloma cells P3U1 using polyethylene glycol 4000 (Merck). Hybridomas were selected by growth on S-Clon cloning medium (Adia Co., Ltd.) containing hypoxanthine, aminopterin and thymidine. As a result, a plurality of hybridomas were established.
マウス抗ヒトAggrusモノクローナル抗体の分析
フローサイトメトリー解析による検証
 上記のハイブリドーマから得られる抗体のうちMS-1、MS-3およびMS-4という抗体を産生するハイブリドーマを、2011年12月28日に、それぞれ受託番号FERM BP-11447、FERM BP-11448およびFERM BP-11449として独立行政法人 産業技術総合研究所 特許生物寄託センターに寄託した。なお、MS-1、MS-3およびMS-4抗体がヒトAggrusを認識することは、ヒトAggrus遺伝子を導入したCHO細胞株を用いたフローサイトメトリー解析により確認した。具体的には、ヒトAggrus遺伝子を安定的に遺伝子導入したCHO細胞を培養容器から回収し、PBSで洗浄した後2x10 cells/mlの細胞密度に調整したところに、MS-1、MS-3およびMS-4抗体を処理し30分間氷上で反応させた。その後、細胞をPBSで洗浄し2次抗体としてAlexa488標識された抗マウスIgG抗体を処理し氷上で30分間反応させた。細胞をPBSで3回洗浄した後、Cytomics FC500(Beckman Coulter)で解析を行った。解析結果を図12に示す。 Analysis of mouse anti-human Aggrus monoclonal antibody
Verification by Flow Cytometry Analysis Among the antibodies obtained from the above hybridomas, hybridomas producing the antibodies MS-1, MS-3 and MS-4 were obtained on December 28, 2011, with accession numbers FERM BP-11447, Deposited as FERM BP-11448 and FERM BP-11449 at the National Institute of Advanced Industrial Science and Technology, Patent Biological Depositary. In addition, it was confirmed by flow cytometry analysis using a CHO cell line into which the human Aggrus gene was introduced that the MS-1, MS-3, and MS-4 antibodies recognize human Aggrus. Specifically, CHO cells stably transfected with the human Aggrus gene were collected from the culture vessel, washed with PBS, and adjusted to a cell density of 2 × 10 6 cells / ml. MS-1, MS-3 And MS-4 antibody was treated and reacted on ice for 30 minutes. Thereafter, the cells were washed with PBS, treated with Alexa 488-labeled anti-mouse IgG antibody as a secondary antibody, and reacted on ice for 30 minutes. The cells were washed 3 times with PBS and then analyzed with a Cytomics FC500 (Beckman Coulter). The analysis results are shown in FIG.
エピトープの探索
 ヒトAggrus cDNAからシグナルペプチドに相当するコドンを除去したものをpGEX-6P3ベクターへクローニングし、37から62番目のアミノ酸に相当するコドンをQuickChange Site-Directed Mutagenesis Kit(Stratagene)を用いて1個所ずつアラニンに対応するコドンへと置換することにより、各種アラニン変異型Aggrus発現ベクターを作製した。作製したベクターを用いて大腸菌TOP10F’(Invitrogen)を形質転換して培養した後、大腸菌破砕液をサンプルとしてウェスタンブロット法を行うことにより、組換えヒトAggrusタンパク質に対するP2-0、MS-1、MS-3およびMS-4抗体の反応性を検討した。その結果、図13上段に示されるように、P2-0抗体はヒトAggrusタンパク質の45番目のグリシン、48番目のアスパラギン酸および49番目のアスパラギン酸に対して高い反応性を示し、配列番号1で示すアミノ酸配列を認識することが確認された。MS-1抗体は、ヒトAggrusタンパク質の45番目のグリシンおよび48番目のアスパラギン酸に対して高い反応性を示し、配列番号1で示すアミノ酸配列を認識することが確認された。MS-3抗体は、ヒトAggrusタンパク質の54番目のグリシン、55番目のスレオニンおよび58番目のアスパラギン酸に対して高い反応性を示し、配列番号3で示すアミノ酸配列を認識することが確認された。MS-4抗体は、ヒトAggrusタンパク質の53番目のプロリン、55番目のスレオニン、57番目のグルタミン酸、58番目のアスパラギン酸および61番目のリジンに対して高い反応性を示し、配列番号4で示すアミノ酸配列を認識することが確認された。なお、P2-0、MS-1、MS-3およびMS-4抗体の認識エピトープの模式図を図13下段に示す。ヒトAggrus一次配列中の認識エピトープのうち、白抜き文字で示したアミノ酸が抗体の認識部位であり、楕円と重なる部位は抗体がヒトAggrusを認識する際に重要な領域を示す。 Epitope Search The human Aggrus cDNA from which the codon corresponding to the signal peptide was removed was cloned into the pGEX-6P3 vector. By substituting the codon corresponding to alanine at each site, various alanine mutant Aggrus expression vectors were prepared. After transforming E. coli TOP10F ′ (Invitrogen) using the prepared vector and culturing, Western blotting was carried out using the E. coli disrupted solution as a sample, whereby P2-0, MS-1, and MS against recombinant human Aggrus protein. The reactivity of the -3 and MS-4 antibodies was examined. As a result, as shown in the upper part of FIG. 13, the P2-0 antibody showed high reactivity to the 45th glycine, 48th aspartic acid and 49th aspartic acid of the human Aggrus protein. It was confirmed that the amino acid sequence shown was recognized. The MS-1 antibody was highly reactive to the 45th glycine and 48th aspartic acid of the human Aggrus protein, and was confirmed to recognize the amino acid sequence represented by SEQ ID NO: 1. The MS-3 antibody was highly reactive to the 54th glycine, 55th threonine and 58th aspartic acid of the human Aggrus protein, and was confirmed to recognize the amino acid sequence represented by SEQ ID NO: 3. The MS-4 antibody is highly reactive with the 53rd proline, 55th threonine, 57th glutamic acid, 58th aspartic acid, and 61st lysine of the human Aggrus protein. It was confirmed to recognize the sequence. A schematic diagram of recognition epitopes of P2-0, MS-1, MS-3, and MS-4 antibodies is shown in the lower part of FIG. Among the recognition epitopes in the primary sequence of human Aggrus, the amino acids indicated by white letters are antibody recognition sites, and the region overlapping the ellipse indicates an important region when the antibody recognizes human Aggrus.
表面プラズモン共鳴を用いた組換えヒトAggrusタンパク質に対する抗体の結合度測定
 P2-0、MS-1、MS-3およびMS-4抗体の組換えヒトAggrusタンパク質に対する結合度測定は、表面プラズモン共鳴解析装置Biacore X100(GE Healthcare, Buckinghamshire, UK)を用いた。カルボキシメチルデキストランコート処理が施されたセンサーチップCM5上にアミンカップリング法を用いて組換えヒトAggrusタンパク質を固定化し、約2,000 RU相当の固定化量を得た。25度、30マイクロリットル/minの流速の条件下、HBS-EP+ buffer(10mM HEPES、150mM NaCl、3mM EDTA、0.05% v/v Surfactant P20)を流路に満たして測定を行った。HBS-EP+ bufferを用いてP2-0、MS-1、MS-3およびMS-4抗体溶液を100nM、50nM、25nM、12.5nMおよび6.25nMに各々希釈し、組換えヒトAggrusタンパク質が固定化されたセンサーチップCM5上に60秒間流して結合反応を観察し、引き続きHBS-EP+ bufferを120秒間流して解離反応を観察した。測定により得られたセンサーグラムをもとにBiacore X100 evaluation software bivalent analyte modelを用いて解析を行い、解離定数K値を算出した。図14に示されるように、組換えヒトAggrusタンパク質に対するP2-0抗体の解離定数は9.3x10-9 M、MS-1抗体の解離定数は9.0x10-9 M、MS-3抗体の解離定数は6.3x10-8 M、MS-4抗体の解離定数は2.0x10-6 Mであった。 Measurement of binding degree of antibody to recombinant human Aggrus protein using surface plasmon resonance Measurement of binding degree of P2-0, MS-1, MS-3 and MS-4 antibodies to recombinant human Aggrus protein is a surface plasmon resonance analyzer. Biacore X100 (GE Healthcare, Buckinghamshire, UK) was used. Recombinant human Aggrus protein was immobilized on sensor chip CM5 that had been subjected to carboxymethyl dextran coating treatment using an amine coupling method to obtain an immobilized amount equivalent to about 2,000 RU. Measurement was performed by filling the flow path with HBS-EP + buffer (10 mM HEPES, 150 mM NaCl, 3 mM EDTA, 0.05% v / v Surfactant P20) under the conditions of a flow rate of 25 degrees and 30 microliters / min. Dilute P2-0, MS-1, MS-3 and MS-4 antibody solutions to 100 nM, 50 nM, 25 nM, 12.5 nM and 6.25 nM, respectively, using HBS-EP + buffer to fix the recombinant human Aggrus protein The binding reaction was observed by flowing for 60 seconds on the converted sensor chip CM5, and then the dissociation reaction was observed by flowing HBS-EP + buffer for 120 seconds. The sensorgrams obtained by measurement analyzed using based on Biacore X100 evaluation software bivalent analyte model, to calculate the dissociation constant K D values. As shown in FIG. 14, the dissociation constant of P2-0 antibody against recombinant human Aggrus protein is 9.3 × 10 −9 M, the dissociation constant of MS-1 antibody is 9.0 × 10 −9 M, and the dissociation of MS-3 antibody The constant was 6.3 × 10 −8 M, and the dissociation constant of the MS-4 antibody was 2.0 × 10 −6 M.
Aggrus-CLEC-2結合阻害試験
 哺乳動物細胞から精製した組換えAggrusタンパク質およびCLEC-2タンパク質を用いて、Aggrus-CLEC-2相互作用をELISA法により検出した。また、抗Aggrus抗体がAggrus-CLEC-2相互作用に与える影響を検討した。図15上段に示されるように、P2-0およびMS-1抗体は、処理濃度依存的にAggrus-CLEC-2相互作用を阻害することが示された。また、図15下段に示されるように、MS-3およびMS-4抗体は40マイクログラム/mlもしくは80マイクログラム/mlと高濃度で処理することにより、Aggrus-CLEC-2相互作用を阻害することが示された。 Aggrus-CLEC-2 binding inhibition test Aggrus-CLEC-2 interaction was detected by ELISA using recombinant Aggrus protein and CLEC-2 protein purified from mammalian cells. In addition, the effect of the anti-Aggrus antibody on the Aggrus-CLEC-2 interaction was examined. As shown in the upper part of FIG. 15, P2-0 and MS-1 antibodies were shown to inhibit the Aggrus-CLEC-2 interaction in a treatment concentration-dependent manner. In addition, as shown in the lower part of FIG. 15, the MS-3 and MS-4 antibodies inhibit the Aggrus-CLEC-2 interaction by treating at a high concentration of 40 microgram / ml or 80 microgram / ml. It was shown that.
血小板凝集抑制試験
 血小板凝集を引き起こさない細胞株であるCHO細胞にヒトAggrus遺伝子を導入すれば、血小板凝集を引き起こすようになることが知られている。MCM HEMA TRACER 313M(エム・シー・メディカル)を用いた光透過率のモニタリングによるin vitro血小板凝集分析を行い、反応開始時点から最大凝集率の50%に至るまでの時間を比較した。図16に示されるように、ヒトAggrus導入CHO細胞により誘導される血小板凝集は、コントロール抗体(マウスIgG(Sigma社カタログ番号I5381をPBS透析したもの))存在下では反応開始から2~3.5分で50%凝集率に到達するのに対し、P2-0抗体存在下では反応開始から11~19分後に遅延した。また、MS-1抗体存在下では、反応開始から9分後、MS-3抗体存在下では反応開始から14.5分後、MS-4抗体存在下では反応開始から10分後に遅延した。このことから、P2-0、MS-1、MS-3およびMS-4抗体はAggrus依存的な血小板凝集を阻害する活性を有することが示された。 Platelet Aggregation Inhibition Test It is known that the introduction of a human Aggrus gene into CHO cells, which are cell lines that do not cause platelet aggregation, causes platelet aggregation. In vitro platelet aggregation analysis was performed by monitoring light transmittance using MCM HEMA TRACER 313M (MC Medical), and the time from the start of the reaction to 50% of the maximum aggregation rate was compared. As shown in FIG. 16, platelet aggregation induced by human Aggrus-introduced CHO cells is 2 to 3.5 from the start of the reaction in the presence of a control antibody (mouse IgG (Sigma catalog number I5381 obtained by PBS dialysis)). The 50% aggregation rate was reached in minutes, whereas in the presence of the P2-0 antibody, the reaction was delayed 11 to 19 minutes after the start of the reaction. In the presence of MS-1 antibody, the reaction was delayed 9 minutes after the start of the reaction, in the presence of MS-3 antibody, 14.5 minutes after the start of the reaction, and in the presence of MS-4 antibody, the reaction was delayed 10 minutes after the start of the reaction. From this, it was shown that P2-0, MS-1, MS-3 and MS-4 antibodies have an activity of inhibiting Aggrus-dependent platelet aggregation.
抗腫瘍活性試験
 BALB/c-nu/nuヌードマウス12匹の背部皮下にヒトAggrus遺伝子を導入したCHO細胞株を1x10 cells/匹の細胞数で移植し、6匹2群にわけた。細胞移植を行った日をDay0とし、Day1、Day5およびDay9の合計3回にわたりコントロール抗体(マウスIgG2a(Sigma社カタログ番号M9144をPBS透析したもの))およびMS-1抗体を各群に投与した。なお、1回の抗体投与量は30マイクログラム/匹とし、投与経路には尾静脈を採用した。腫瘍体積を1週間に2回測定し、皮下移植から30日後まで測定することにより、MS-1抗体の抗腫瘍効果を検討した。その結果、図17のグラフに示されるように、コントロール抗体投与群では6匹中5匹のマウスにおいて腫瘍の増殖が観察され、Day30における平均腫瘍体積は約1200mmであった。一方、MS-1抗体投与群では6匹中2匹のマウスにおいて腫瘍の消失、3匹のマウスにおいて腫瘍の増殖抑制が観察され、Day30における平均腫瘍体積は400mmであった。このことから、MS-1抗体はヒトAggrus発現細胞に対して抗腫瘍活性を発揮することが示された。なお、Day18におけるマウスと腫瘍の様子を図17右側に写真で示す。マウスに記された1から6までの数字は、各グラフの1から6までの凡例に対応している。 Anti-tumor activity test CHO cell line into which human Aggrus gene was introduced was subcutaneously implanted into the back of 12 BALB / c-nu / nu nude mice at a cell number of 1 × 10 5 cells / mouse and divided into 2 groups of 6 mice. The day of cell transplantation was set to Day 0, and a control antibody (mouse IgG2a (Sigma catalog number M9144 dialyzed with PBS)) and MS-1 antibody were administered to each group three times in total, Day1, Day5 and Day9. In addition, the dose of one antibody was 30 microgram / animal, and the tail vein was adopted as the administration route. The tumor volume was measured twice a week and the antitumor effect of the MS-1 antibody was examined by measuring until 30 days after subcutaneous implantation. As a result, as shown in the graph of FIG. 17, tumor growth was observed in 5 out of 6 mice in the control antibody administration group, and the average tumor volume at Day 30 was about 1200 mm 3 . On the other hand, in the MS-1 antibody administration group, tumor disappearance was observed in 2 out of 6 mice, and growth inhibition of tumor was observed in 3 mice, and the average tumor volume in Day 30 was 400 mm 3 . From this, it was shown that MS-1 antibody exhibits antitumor activity against human Aggrus-expressing cells. The state of mice and tumors on Day 18 is shown on the right side of FIG. The numbers from 1 to 6 marked on the mouse correspond to the legends from 1 to 6 in each graph.
肺への自然転移阻害試験
 ヒトAggrusを導入したCHO細胞を皮下移植した場合、移植後30日程度で肺への自然転移が観察されることが知られている。そこで、抗腫瘍活性試験を実施した12匹のマウスの肺を細胞移植後30日目に摘出し、PBS洗浄後に飽和ピクリン酸溶液で染色し、肺表面に生じた転移結節数をカウントした。図18上側にカウントした転移結節数を記したグラフを、下側にピクリン酸染色したマウスの肺の写真を示す。コントロール抗体(マウスIgG2a(Sigma社カタログ番号M9144をPBS透析したもの))投与群では平均30個程度の肺転移結節が観察されたのに対し、MS-1抗体投与群では6匹中5匹において肺転移結節の形成が完全に阻害された。このことから、MS-1抗体はヒトAggrus依存的な肺への自然転移を阻害する活性を有していることが示された。 Spontaneous Metastasis Inhibition Test to Lung It is known that when CHO cells introduced with human Aggrus are subcutaneously transplanted, spontaneous metastasis to the lung is observed about 30 days after transplantation. Therefore, lungs of 12 mice subjected to the antitumor activity test were excised 30 days after cell transplantation, washed with PBS and stained with a saturated picric acid solution, and the number of metastatic nodules generated on the lung surface was counted. FIG. 18 shows a graph showing the number of metastatic nodules counted on the upper side, and a photograph of a mouse lung stained with picric acid on the lower side. In the control antibody (mouse IgG2a (Sigma catalog No. M9144 dialyzed with PBS)) group, an average of about 30 lung metastatic nodules were observed, whereas in the MS-1 antibody group, 5 out of 6 mice were observed. The formation of lung metastatic nodules was completely inhibited. From this, it was shown that the MS-1 antibody has an activity to inhibit human Aggrus-dependent spontaneous lung metastasis.
肺転移抑制試験
 ヒトAggrusを導入したCHO細胞をBALB/c-nu/nuヌードマウスの尾静脈より注射すると、約20日後に肺転移結節を形成することが知られている。そこで、細胞注射の前日にコントロール抗体(マウスIgG2a(Sigma社カタログ番号M9144をPBS透析したもの))、MS-1抗体およびMS-3抗体を尾静脈経路で各群8匹のヌードマウスに投与し、Aggrus依存的な実験的肺転移に与える影響を検討した。図19に示されるように、MS-1およびMS-3抗体を事前投与することにより、濃度依存的にヒトAggrus導入CHO細胞の肺転移が顕著に抑制された。従って、MS-1およびMS-3抗体はAggrus中和活性があるだけでなく、Aggrus依存的な血行性転移を阻害することも示された。 Lung Metastasis Inhibition Test It is known that when CHO cells introduced with human Aggrus are injected from the tail vein of BALB / c-nu / nu nude mice, lung metastasis nodules are formed about 20 days later. Therefore, the control antibody (mouse IgG2a (Sigma catalog number M9144 dialyzed in PBS)), MS-1 antibody and MS-3 antibody were administered to 8 nude mice in each group via the tail vein route the day before cell injection. The effect on Aggrus-dependent experimental lung metastasis was examined. As shown in FIG. 19, lung metastasis of human Aggrus-introduced CHO cells was remarkably suppressed in a concentration-dependent manner by pre-administration with MS-1 and MS-3 antibodies. Thus, MS-1 and MS-3 antibodies were shown not only to have Aggrus neutralizing activity but also to inhibit Aggrus-dependent hematogenous metastasis.
FERM BP-11446
FERM BP-11447
FERM BP-11448
FERM BP-11449 FERM BP-11446
FERM BP-11447
FERM BP-11448
FERM BP-11449

Claims (9)

  1.  配列番号1、3又は4により表されるアミノ酸配列からなるAggrusのエピトープを認識する、マウスモノクローナル抗体又はその機能的断片からなるフラグメント。 A fragment consisting of a mouse monoclonal antibody or a functional fragment thereof that recognizes an Agrus epitope consisting of the amino acid sequence represented by SEQ ID NO: 1, 3, or 4.
  2.  受託番号FERM BP-11446、FERM BP-11447、FERM BP-11448又はFERM BP-11449のハイブリドーマにより産生される、請求項1記載のモノクローナル抗体又はその機能的断片からなるフラグメント。 The fragment consisting of the monoclonal antibody or the functional fragment thereof according to claim 1, which is produced by a hybridoma having a deposit number of FERM BP-11446, FERM BP-11447, FERM BP-11448 or FERM BP-11449.
  3.  ヒト化された、請求項1又は2記載のモノクローナル抗体又はその機能的断片からなるフラグメント。 A humanized fragment comprising the monoclonal antibody or functional fragment thereof according to claim 1 or 2.
  4.  受託番号FERM BP-11446、FERM BP-11447、FERM BP-11448又はFERM BP-11449のハイブリドーマ。 Hybridomas with accession numbers FERM BP-11446, FERM BP-11447, FERM BP-11448 or FERM BP-11449.
  5.  請求項1~3のいずれか一項記載のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、Aggrus-CLEC-2結合阻害剤。 An Aggrus-CLEC-2 binding inhibitor comprising the monoclonal antibody according to any one of claims 1 to 3 or a fragment comprising a functional fragment thereof.
  6.  血小板凝集抑制又は癌転移抑制、あるいは腫瘍又は血栓症の処置のための、請求項1~3のいずれか一項記載のモノクローナル抗体又はその機能的断片からなるフラグメントを含む、医薬組成物。 A pharmaceutical composition comprising a monoclonal antibody or a fragment comprising a functional fragment thereof according to any one of claims 1 to 3, for inhibiting platelet aggregation, inhibiting cancer metastasis, or treating a tumor or thrombosis.
  7.  血栓症が、脳梗塞又は心筋梗塞である、請求項6記載の医薬組成物。 The pharmaceutical composition according to claim 6, wherein the thrombosis is cerebral infarction or myocardial infarction.
  8.  癌又は腫瘍が、扁平上皮癌、繊維肉腫、中皮腫、カポジ肉腫、精巣腫瘍、脳腫瘍又は膀胱癌である、請求項6記載の医薬組成物。 The pharmaceutical composition according to claim 6, wherein the cancer or tumor is squamous cell carcinoma, fibrosarcoma, mesothelioma, Kaposi sarcoma, testicular tumor, brain tumor or bladder cancer.
  9.  癌又は腫瘍が、扁平上皮癌、中皮腫、精巣腫瘍又は膀胱癌である、請求項8記載の医薬組成物。 The pharmaceutical composition according to claim 8, wherein the cancer or tumor is squamous cell carcinoma, mesothelioma, testicular tumor or bladder cancer.
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WO2015053381A1 (en) * 2013-10-10 2015-04-16 幸成 加藤 Anti-podoplanin antibody
JPWO2015053381A1 (en) * 2013-10-10 2017-03-09 株式会社ペルセウスプロテオミクス Anti-podopranin antibody
US10227407B2 (en) 2013-10-10 2019-03-12 Yukinari Kato Anti-podoplanin antibody
WO2017010463A1 (en) * 2015-07-15 2017-01-19 公益財団法人がん研究会 Anti-aggrus monoclonal antibody, domain in aggrus which is required for binding to clec-2, and method for screening for aggrus-clec-2 binding inhibitor
JPWO2017010463A1 (en) * 2015-07-15 2018-07-05 公益財団法人がん研究会 Screening method for anti-Aggrus monoclonal antibody, region of Aggrus required for binding to CLEC-2, and Aggrus-CLEC-2 binding inhibitor
EP3323831A4 (en) * 2015-07-15 2019-02-27 Japanese Foundation For Cancer Research Anti-aggrus monoclonal antibody, domain in aggrus which is required for binding to clec-2, and method for screening for aggrus-clec-2 binding inhibitor
US10730939B2 (en) 2015-07-15 2020-08-04 Japanese Foundation For Cancer Research Anti-Aggrus monoclonal antibody, domain in Aggrus which is required for binding to CLEC-2, and method for screening for Aggrus-CLEC-2 binding inhibitor
JP2021046417A (en) * 2015-07-15 2021-03-25 公益財団法人がん研究会 Anti-aggrus monoclonal antibodies, regions of aggrus necessary for binding to clec-2 and methods for screening inhibitors of aggrus-clec-2 binding
JP7122361B2 (en) 2015-07-15 2022-08-19 公益財団法人がん研究会 Anti-Aggrus Monoclonal Antibodies, Regions of Aggrus Required for CLEC-2 Binding, and Screening Methods for Aggrus-CLEC-2 Binding Inhibitors
WO2019081714A1 (en) 2017-10-26 2019-05-02 Vib Vzw Podoplanin positive macrophages
WO2022154045A1 (en) * 2021-01-13 2022-07-21 株式会社Lsiメディエンス Method for predicting risk for thrombosis in cancer patient using soluble clec2

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EP2690111A1 (en) 2014-01-29
JPWO2012128082A1 (en) 2014-07-24
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ES2566133T3 (en) 2016-04-11
CN104093741B (en) 2016-12-07
US20140235827A1 (en) 2014-08-21
KR20140053873A (en) 2014-05-08
EP2690111A4 (en) 2014-12-31
EP2690111B1 (en) 2016-03-09
JP6218603B2 (en) 2017-10-25

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